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Optimisation of an asymmetric polymerase chain reaction assay for the amplification of single-stranded DNA from Wuchereria bancrofti for electrochemical detection

机译:不对称聚合酶链反应分析法的优化,用于扩增班氏无节菌单链DNA进行电化学检测

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Single-stranded DNA (ssDNA) is a prerequisite for electrochemical sensor-based detection of parasite DNA and other diagnostic applications. To achieve this detection, an asymmetric polymerase chain reaction method was optimised. This method facilitates amplification of ssDNA from the human lymphatic filarial parasite Wuchereria bancrofti. This procedure produced ssDNA fragments of 188 bp in a single step when primer pairs (forward and reverse) were used at a 100:1 molar ratio in the presence of double-stranded template DNA. The ssDNA thus produced was suitable for immobilisation as probe onto the surface of an Indium tin oxide electrode and hybridisation in a system for sequence-specific electrochemical detection of W. bancrofti. The hybridisation of the ssDNA probe and target ssDNA led to considerable decreases in both the anodic and the cathodic currents of the system's redox couple compared with the unhybridised DNA and could be detected via cyclic voltammetry. This method is reproducible and avoids many of the difficulties encountered by conventional methods of filarial parasite DNA detection; thus, it has potential in xenomonitoring.
机译:单链DNA(ssDNA)是基于电化学传感器的寄生虫DNA检测和其他诊断应用的先决条件。为了实现该检测,对不对称聚合酶链反应方法进行了优化。该方法有助于从人淋巴丝状寄生虫Wuchereria bancrofti扩增ssDNA。当在双链模板DNA存在的情况下以100:1的摩尔比使用引物对(正向和反向)时,此步骤可一步生成188 bp的ssDNA片段。由此产生的ssDNA适合于作为探针固定在氧化铟锡电极的表面上,并且适合在用于班氏罗非鱼的序列特异性电化学检测的系统中杂交。与未杂交的DNA相比,ssDNA探针与目标ssDNA的杂交导致系统氧化还原对的阳极和阴极电流显着降低,可以通过循环伏安法检测到。该方法可重现,避免了常规的丝虫寄生虫DNA检测方法所遇到的许多困难;因此,它具有异种监测的潜力。

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